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General Transfection

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Introduction

This protocol describes a general method for transfecting mammalian cells using linear polyethylenimine. Transfections allow for transient expression of a gene of interest in a target cell line and can be useful for short term studies of protein function. We specifically use this protocol with Lenti-X 293T cells, a cell line optimized for production of lentiviral vectors. This approach can be adapted for different cell lines and different transfection reagents.

Last Upload: June 10, 2016

Workflow Timeline

Day 0: Seed Lenti-X 293T cells (this cell line is optimized for production of lentiviral vectors)

Reagent Preparation

*Pro-Tips* Different brands and lots of FBS can promote or inhibit transfection. Test a variety of brands and lots of FBS to find one suitable with your protocols.FBS can be purchased already head inactivated or it can be inactivated in the lab by heating to 56 ℃ for 30 minutes.

Aliquots can be thawed and stored at 4 ℃ prior to use. Thawed aliquots should be discarded after 1-2 months.

1 mg/mL polyethylenimine, linear MW 25,000 Da (PEI)

Dissolve 100 mg of powder into 100 mL of deionized water.

While stirring, slowly add hydrochloric acid until the solution clears.

Check the pH of the solution

Use hydrochloric acid or sodium hydroxide to adjust the pH to 7.0. Typically the solution will be basic and will need adjustment with hydrochloric acid first.

*Pro-Tip* The pH of this solution will drift pretty rapidly upon addition of acid or base. Add only a few drops at a time, allow them to mix and recheck the pH to prevent over or undershooting the desired pH.

Allow the solution to mix for 10 min and then recheck the pH to ensure that it has not drifted.

Filter the solution through a 0.22 um membrane.

Aliquot 500-1000 ul into sterile tubes.

Store the tubes at -80 ℃.

After thawing the solution can be stored at 4 ℃ for up to 2 months. After 2 months, discard the tube and thaw a new working stock.

Considerations Before You Start

The health of the packaging cell line is critical for obtaining high levels of virus.

Lenti-X 293T cells should be split 3 times a week:

Monday: Plate 1x106 cells in a 75 cm2 flask in a volume of 15 mL.

Wednesday: Plate 1x106 cells in a T75 flask in a volume of 15 mL.

Friday: Plate 8x105 cells in a T75 flask in a volume of 15 mL.

Do not add antibiotics to the media.

Use cells that are below passage 15 for viral production.

The optimal mass DNA:mass PEI ratio will need to be empirically determined for each new batch of 1 mg/mL PEI prepared.

There may be variation between batches of PEI depending on the user, quantities of chemical used, volumes, pH adjustment etc. Consequently, each batch needs to be validated and the best ratio of mass DNA:mass PEI determined.

*Pro-Tip* Endotoxins can inhibit transfection, therefore, plasmid DNA purification should include an endotoxin removal step. For high quality plasmid DNA, the plasmid should also be propagated in an endonuclease negative E. coli strain such as NEB stable.

*Pro-Tip* The ratio of ug DNA:ug PEI needs to be empirically determined. Once a batch of PEI is prepared, transfect cells with a fluorescent plasmid using a variety of ratios. Check the cells 1-2 days after transfection to determine what ratio gives the highest percentage of GFP positive cells.

Carefully transfer the transfection mix to the Lenti-X 293T packaging cells. Add the transfection mix dropwise being careful not to dislodge the cells.

Incubate the cells for 18 h, or until the following morning.

The following morning, carefully aspirate the media. Replace the media with 15 mL of DMEM complete.

Incubate the cells 24-48 h before checking for protein expression.

Sample Data

Legend: Lenti-X 293T cells were transfected using 1:1, 1:2, 1:3 and 1:6 ug of pRosetta:ug of PEI. The 1:2 and 1:3 ratios provided high transfection efficiencies as can be seen here by the amount of green fluorescent protein expression (green in the right panels) with a limited effect on cell growth.